Transcription of Spectrophotometric Nucleic Acid Quantification
1 Spectrophotometric Nucleic acid Quantification in Microplates and Micro-Volumes Application GuideBioTek Instruments, Box 998, Highland Park, Winooski, Vermont 05404-0998 USAP hone: 888-451-5171 Outside the USA: 802-655-4740 Email: 2012 Why Quantify Nucleic Acids? Nucleic acids are the building blocks of life in all living things, from plants and animals to bacteria and viruses. In research, it s important to quantify RNA and DNA prior to downstream processes like sequenc-ing, restriction enzyme digestions and ligations, PCR and qPCR along with many other applications. Along with determining Nucleic acid concentrations, it s also important to calculate the ratio of Nucleic acid to protein to ascertain purity before using the sample in downstream applications.
2 There are fluorometric and Spectrophotometric methods for Nucleic acid Quantification . The former is used for applications requiring high sensitivity due to minute available amounts of Nucleic acid ; the latter is more conventionally used from common Nucleic acid extraction procedures. In this application guide, we ll discuss in detail the Spectrophotometric methodology as performed in microplate instrumentation and in specialized micro-volume accessories. Absorbance Quantification MethodsNucleic acid Quantification is commonly performed in a cuvette spectrophotometer, where the mono-chromator optical system provides light at 260 nm, the absorbance peak for DNA and RNA. Increas-ingly, microplate spectrophotometers are being used to quantify Nucleic acids as well due to increased sample absorbed by the Nucleic acid in the sample correlates to the concentration of Nucleic acid present.
3 Both DNA and RNA absorb light at 260 nm, therefore this is a measurement of total Nucleic acid . Nucleic acid samples are also typically measured at 280 nm, which is the absorbance peak for protein. The ratio of the 260 nm and 280 nm measurements provides a determination of the purity of the Nucleic acid , with a ratio near 2 indicating a highly pure Nucleic acid sample. (Fig. 1) Figure 1. Typical absorbance spectrum for DNA, RNA and protein, indicating the peak at about 260 nm for DNA and RNA and the peak at about 280 nm for and other Sample Vessel TypesA cuvette-based spectrophotometer has a horizontal light path where the wavelength-specific light is perpendicular to the sample.
4 Most standard cuvettes have fixed optical path lengths of 1 cm. A microplate spectrophotometer, measures samples in a microplate, therefore the light path is vertical and varies according to the volume in the microplate well. (Fig. 2) 2 Application GuideNucleic acid QuantificationFigure 2. Comparison of the fixed 1 cm path length of light in a cuvette based system and the variable vertical light path of a microplate based SourceDetectorCuvetteMicrowellAbsorbing SolutionThe advantage of a cuvette-based method is that it is simple and precise, while the disadvantages include limited throughput of one-at-a-time sample measurements and the need to dilute samples. BioTek offers the patented BioCell , a sample cuvette with a fixed 1 cm path length that can be measured in a microplate spectrophotometer and offers the advantages of a traditional cuvette spectrophotometer.
5 (Fig. 3) Figure 3. BioTek s patented BioCell allows fixed 1 cm path length readings in most of BioTek s microplate spectrophotometers. Up to 8 BioCells can be measured at a spectrophotometers and some micro-volume systems offer multiple sample throughput and in some cases, sample dilution may not be convention, the extinction coefficients for Nucleic acids and protein are based on a 1 cm path length (Table 1). There-fore, in a microplate spectrophotometer, where the sample path length is dependent upon the volume in the microplate well, it is necessary to correct the path length of the sample to a 1 cm equivalent in order to proceed to quantify the sample. Nucleic acid TypeAverage Extinction Coefficient ( g/mL)-1 cm-1 Concentration ( g/mL) if OD=1*Double-stranded 1.
6 Commonly accepted extinction coefficients at known concentration.* Based on a 1 cm path GuideNucleic acid QuantificationPath Length Correction and Nucleic acid QuantificationNucleic acid calculations are based on the Beer-Lambert Law, credited to the separate research of August Beer and Johann Heinrich Lambert in the 19th and 18th centuries, respectively. The Beer-Lambert equation is shown here:OD= Cb According to this equation, the optical density (OD) of the sample can be found by the product of the extinction coef-ficient ( ) and concentration (C) of the sample and path length (b) of the measuring microplate spectrophotometers, the OD measurement is taken vertically through the samples in the plate, and there-fore the path length of the samples will vary according to the volume in the well.
7 To correct the path length to 1 cm, BioTek s reader control and data analysis software, Gen5 , has a built-in method for samples diluted in water. Gen5 s method uses the absorbance peak of water at room temperature (977 nm), and a blank measurement of 900 nm. The 977 nm 900 nm optical density difference is divided by , which is the known optical density for water at 1 cm. The result of this calculation is the path length of the sample, which can then be used to cal-culate the concentration of Nucleic acid in the microplate wells. A step-wide procedure contained in the Gen5 method appears below:The latest methods for Nucleic acid Quantification use very low volume samples, typically 2 L or less, to conserve pre-cious samples and reagents.
8 BioTek s Take3 or Take3 Trio Micro-Volume plate can be read in a BioTek microplate spectrophotometer to measure multiple Nucleic acid samples and provide quick Quantification results. The Take3 plates use a quartz slide with a hydrophobic coating to create microspots suitable for 2 L samples. (Fig. 5) When the plate lid is closed, the samples are sandwiched between the two surfaces in a fixed nominal mm path length. This very short path length allows high concentration of Nucleic acids to be measured without dilution. After each measurement, the slides can be easily wiped clean and reused. BioTek s automated method of path length correction and Quantification (dsDNA example): 1.
9 Measure the OD of the solution at 977 nm 900 nm, then divide by the known OD of water @ 1 cm: A977 A900 sample / OD = sample path length (in cm) 2. Measure the sample at 260 nm (minus a blank) and divide by the path length: A260 sample A260 blank / sample path length = OD corrected to 1 cm 3. To calculate the concentration of DNA in the sample wells, multiply the corrected OD values by the extinction coefficient: OD corrected to 1 cm * 50 = concentration of DNA in the well (in g/mL)4 Application GuideNucleic acid QuantificationNucleic acid PurityAlong with the calculation of Nucleic acid concentration, it is important to determine the purity of the sample prior to downstream applications.
10 Proteins and other contaminants like phenol and salts associated with the extraction process may interfere with true values and skew results. Purity of Nucleic acid samples is determined by finding the ratio of the Nucleic acid measurement at 260 nm and the protein measurement at 280 nm, where protein absorbance peaks. To cor-rect for background turbidity, a measurement at about 320 nm can also be taken, since protein and Nucleic acids do not absorb light at this wavelength. This ratio calculation and background subtraction is typically done automatically in the systems described in this A260 / A280 ratio is an approximation of purity that will approach the ideal ratios shown in Table 2, but it is not an ab-solute value.